Chen Hauh-Jyun Candy, Chen Yu-Chin, Hsiao Chiung-Fong, Chen Pin-Fan
Department of Chemistry and Biochemistry, National Chung Cheng University , 168 University Road, Ming-Hsiung, Chia-Yi 62142, Taiwan.
Buddhist Dalin Tzu Chi General Hospital , No.2, Minsheng Road, Dalin, Chia-Yi 622, Taiwan.
Chem Res Toxicol. 2015 Dec 21;28(12):2377-89. doi: 10.1021/acs.chemrestox.5b00380. Epub 2015 Nov 10.
Glyoxal and methylglyoxal are oxoaldehydes derived from the degradation of glucose-protein conjugates and from lipid peroxidation, and they are also present in the environment. This study investigated the site-specific reaction of glyoxal and methylglyoxal with the amino acid residues on human hemoglobin using a shot-gun proteomic approach with nanoflow liquid chromatography/nanospray ionization tandem mass spectrometry (nanoLC-NSI/MS/MS). In human hemoglobin incubated with glyoxal, modification on 8 different sites, including lysine residues at α-Lys-11, α-Lys-16, α-Lys-56, β-Lys-17, β-Lys-66, β-Lys-144, and arginine residues at α-Arg-92 and β-Arg-30, was observed using a data-dependent scan. In methylglyoxal-treated hemoglobin, there were specific residues, namely, α-Arg-92, β-Lys-66, β-Arg-30, and β-Lys-144, forming carboxyethylation as well as the dehydrated product hydroimidazolone at α-Arg-92 and β-Arg-30. These lysine and arginine modifications were confirmed by accurate mass measurement and the MS(2) and MS(3) spectra. The most intensive signal of each modified peptide was used as the precursor ion to perform the product ion scan. The relative extent of modifications was semiquantified simultaneously relative to the native reference peptide by nanoLC-NSI/MS/MS under the selected reaction monitoring (SRM) mode. The extent of these modifications increased dose-dependently with increasing concentrations of glyoxal or methylglyoxal. Six out of the eight modifications induced by glyoxal and three out of the six modifications induced by methylglyoxal were detected in hemoglobin freshly isolated from human blood samples. The relative extent of modification of these post-translational modifications was quantified in poorly controlled type 2 diabetes mellitus patients (n = 20) and in nondiabetic control subjects (n = 21). The results show that the carboxymethylated peptides at α-Lys-16, α-Arg-92, β-Lys-17, β-Lys-66, and the peptide at α-Arg-92 with methylglyoxal-derived hydroimidazolone are significantly higher in diabetic patients than in normal individuals (p value <0.05). This report identified and quantified glyoxal- and methylglyoxal-modified hemoglobin peptides in humans and revealed the association of the extent of modifications at specific sites with T2DM. Only one drop (10 μL) of fresh blood is needed for this assay, and only an equivalent of 1 μg of hemoglobin was analyzed by the nanoLC-NSI/MS/MS-SRM system. These results suggest the potential use of these specific post-translational modifications in hemoglobin as feasible biomarker candidates to assess protein damage induced by glyoxal and methylglyoxal.
乙二醛和甲基乙二醛是由葡萄糖 - 蛋白质共轭物降解以及脂质过氧化产生的氧代醛,它们也存在于环境中。本研究采用纳流液相色谱/纳喷雾电离串联质谱(nanoLC - NSI/MS/MS)的鸟枪法蛋白质组学方法,研究了乙二醛和甲基乙二醛与人血红蛋白上氨基酸残基的位点特异性反应。在用乙二醛孵育的人血红蛋白中,使用数据依赖扫描观察到8个不同位点的修饰,包括α - Lys - 11、α - Lys - 16、α - Lys - 56、β - Lys - 17、β - Lys - 66、β - Lys - 144处的赖氨酸残基,以及α - Arg - 92和β - Arg - 30处的精氨酸残基。在经甲基乙二醛处理的血红蛋白中,有特定的残基,即α - Arg - 92、β - Lys - 66、β - Arg - 30和β - Lys - 144,在α - Arg - 92和β - Arg - 30处形成羧乙基化以及脱水产物氢咪唑酮。这些赖氨酸和精氨酸修饰通过精确质量测量以及MS(2)和MS(3)谱得到证实。每个修饰肽的最强信号用作前体离子进行产物离子扫描。在选择反应监测(SRM)模式下,通过nanoLC - NSI/MS/MS相对于天然参考肽同时对修饰的相对程度进行半定量。这些修饰的程度随着乙二醛或甲基乙二醛浓度的增加而呈剂量依赖性增加。在从人血样本中新鲜分离的血红蛋白中检测到乙二醛诱导的8种修饰中的6种以及甲基乙二醛诱导的6种修饰中的3种。在控制不佳的2型糖尿病患者(n = 20)和非糖尿病对照受试者(n = 21)中对这些翻译后修饰的修饰相对程度进行了定量。结果表明,α - Lys - 16、α - Arg - 92、β - Lys - 17、β - Lys - 66处的羧甲基化肽以及含有甲基乙二醛衍生氢咪唑酮的α - Arg - 92处的肽在糖尿病患者中显著高于正常个体(p值<0.05)。本报告鉴定并定量了人体内乙二醛和甲基乙二醛修饰的血红蛋白肽,并揭示了特定位点的修饰程度与2型糖尿病的关联。该检测仅需一滴(10μL)新鲜血液,nanoLC - NSI/MS/MS - SRM系统仅分析了相当于1μg的血红蛋白。这些结果表明,血红蛋白中这些特定的翻译后修饰有可能作为可行的生物标志物候选物,用于评估乙二醛和甲基乙二醛诱导的蛋白质损伤。
